WO1996014406A1 - Method of preparing oligonucleotide probes or primers, vector therefor and use thereof - Google Patents
Method of preparing oligonucleotide probes or primers, vector therefor and use thereof Download PDFInfo
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- WO1996014406A1 WO1996014406A1 PCT/SE1995/001319 SE9501319W WO9614406A1 WO 1996014406 A1 WO1996014406 A1 WO 1996014406A1 SE 9501319 W SE9501319 W SE 9501319W WO 9614406 A1 WO9614406 A1 WO 9614406A1
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- WIPO (PCT)
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- vector
- sequence
- dna fragment
- dna
- restriction enzyme
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
- C12N15/10—Processes for the isolation, preparation or purification of DNA or RNA
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Q—MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
- C12Q1/6844—Nucleic acid amplification reactions
- C12Q1/6853—Nucleic acid amplification reactions using modified primers or templates
- C12Q1/6855—Ligating adaptors
Definitions
- the present invention relates to the preparation of nucleic acid probes and primers as well as vectors therefor.
- the polymerase chain reaction provides a highly efficient method of isolating a desired gene sequence(s) from different DNA samples.
- One general requirement is that sequence information is available from both ends of the fragment to be amplified in order to synthesize specific amplification primers.
- the expense of sequencing DNA and then chemically synthesizing primers still limits the scope of many applications.
- Such genetic markers are required for mapping genetic disease and to establish or extend genetic linkage maps for a variety of organisms.
- RAPD markers serve as a means to establish relatively random polymorphic markers, analyzable by PCR without requiring DNA sequencing and chemical oligonucleotide synthesis of specific primers.
- the present invention provides a different strategy to overcome the deficiences of the prior art methods and permits enzymatic synthesis of specific amplification primers, ligation probes or other probes of known structure but partially unknown sequence without access to clone specific DNA sequence information.
- the invention provides a vector for the preparation of a nucleic acid sequence of known structure but partially unknown sequence, capable of hybridizing to a target DNA sequence without requiring knowledge of this DNA sequence, which vector comprises a site for the insertion of a DNA fragment related to the target DNA sequence, and a recognition sequence for an asymmetrically cleaving restriction enzyme or enzymes on one or both sides of said insertion site.
- the invention provides a method of preparing a nucleic acid sequence of known structure but partially unknown sequence, capable of hybridizing to a target DNA sequence without requiring knowledge of this DNA sequence, which method comprises the steps of ligating or otherwise linking a DNA fragment related to the target sequence to a nucleotide sequence containing the recognition motif of an asymmetrically cleaving restriction enzyme, and subjecting the construct to the restriction enzyme to cleave the construct within the DNA fragment part thereof.
- the invention provides a method for amplifying a DNA fragment without requiring knowledge of the DNA sequence of the fragment by using enzyme-synthesized primers prepared according the above aspect of the invention.
- the invention provides a method for constructing probes for target-dependent ligation reactions.
- Figs. 1A and IB are a schematic representation, in the form of four parts A-D, of a strategy to derive amplification primers enzymatically.
- Part A shows the construction of a specialized cloning vector
- part B shows the cloning of an Alul fragment into the vector
- part C shows enzymatic synthesis of amplification primers
- part D shows amplification of sequences corresponding to those cloned in the vector using primers derived from the amplified insert of the clone.
- the recognition sequences of the restriction enzymes Gsul and Alul are highlighted in the figures.
- Fig. 2 is a schematic representation of an immobilized vector containing a Gsul site, the cleavage thereof to prepare a circularizable probe, and the use of the latter for the capture and subsequent release of single-stranded circular target molecules.
- Fig. 3 is a photograph of an autoradiograph of a comparison of amplification products obtained by PCR using sets of primers derived by solid-phase chemical synthesis or enzymatically.
- specific 16-mer primers that were synthesized by standard solid phase chemistry, were compared with similarly constructed 38-mer primers of the same 16-base sequence at the 3 '-end, and with an enzymatically synthesized primer pair, expected to have the same 38-mer sequence as the chemically synthesized oligonucleotides of this size.
- restriction endonuclease is an enzyme capable of recognizing a specific DNA sequence (usually four to eight nucleotides in sequence) and cleaving the DNA, thereby creating double-stranded breaks.
- the restriction enzymes are grouped into four classes, type I, II, III and IV, on the basis of their subunit structure, cofactor requirements, substrate specificity and several other features.
- Type I enzymes cleave the substrate DNA almost at random at a great distance from the recognition site.
- Type II enzymes exemplified by EcoRI, cleave within the recognition site or a few nucleotides away. Both type
- Type IV enzymes cleave the target DNA sequence some considerable distance away from the recognition site and they also have in common the property of never cleaving the DNA to completion.
- Type IV enzymes differ from the type III enzymes in that they, similar to the type II restriction enzymes, are not dependent upon ATP. The type III and type
- IV restriction enzymes are commonly called asymmetrically cleaving enzymes.
- Exemplary of type IV restriction enzymes are Gsul (Janulaitis et al., Nucl. Acid Res. 1989; 17(14) :1989) , with the recognition motif 5'CTGGAG3' and cleaving 16 bases downstream of this motif; Eco57l, with the recognition sequence 5'CTGGTG3' and cleaving 16 bases downstream of this motif; Mmel (Boyd et al., Nucl. Acid Res. 1986; 17 (14) :5255-5274, with a 6-base recognition motif, and which cleaves the target DNA 22 bases downstream of this sequence.
- Restriction enzyme Bpml (available from New England Biolabs, U.S.A.) has the same recognition sequence and cleaves in the same way as Gsul above.
- type III or IV enzymes cleaving the target DNA even farther from the recognition sequence. Examples of such enzymes include Ecol5 and HinP151 cleaving 25 or 26 bases downstream of the recognition sequence.
- the property of type III or IV restriction enzymes to cleave asymmetrically, i.e. to cleave a DNA substrate at a distance from the recognition sequence is utilized to prepare probes or primers of a defined size capable of hybridizing to a target DNA sequence without a requirement to know this DNA sequence.
- amplification primers are prepared which may then be used, optionally in combination with a standard vector sequence-derived oligonucleotide, for amplification to large copy numbers, starting from a genomic DNA sample.
- defined size amplification primers may be produced enzymatically through digestion inside the cloned fragments in amplif i cation products by locating a recognition sequence for an asymmetrically cleaving restriction enzyme on both sides of the cloning site.
- the digestion is independent of the DNA sequence of the cloned fragment, and the cleavage products consisting of the original amplification primers having linked thereto a respective part of the cloned DNA fragment may be used to amplify sequences corresponding to the cloned DNA fragment from er DNA samples.
- a plasmid vector is cleaved at a desired site, and an oligonucleotide duplex, or linker, containing the recognition site for an asymmetrically cleaving restriction enzyme, in the figure by way of example the recognition motif for Gsul, is ligated to each vector fragment end.
- Both linkers lack 5'- phosphate groups to prevent them from ligating to themselves. Ligation of linkers to the restriction fragment ends does not recreate the restriction site, so that over time more and more restriction ends are modified with linker dimers.
- the vector produced is then isolated, e.g. by gel purification, from remaining circular vector molecules and used for molecular cloning of DNA fragments. This is schematically illustrated in Fig. 1A, part B which shows the construction of a recombinant molecule by ligating a blunt end Alul-cleaved DNA-fragment into the vector.
- amplification primers In order to produce amplification primers, individual clones are amplified using a single primer corresponding to one of the linker oligonucleotides and with the 5'-end protected against ⁇ exonuclease digestion, e.g. by a biotin residue at the 5* end.
- the resulting amplification products consist in the cloned Alul-fragment surrounded by vector- derived sequences representing the oligonucleotide dimer ligated to the vector as described above.
- the 6-base motif, 5'CTGGAG3 ' immediately flanking the insert cloned into the vector, represents the recognition sequence for the restriction enzyme Gsul.
- this enzyme cleaves the DNA molecule 16 bases downstream of this motif, inside the fragment cloned into the vector. After digesting the amplification products with this enzyme, the fragments obtained are separated by gel electrophoresis. Thereby the fragments derived from both ends of the amplification product may be quantitated and isolated from remaining undigested or partially digested molecules. Finally, any DNA strands that have 5' phosphate groups are removed by digestion with the enzyme ⁇ exonuclease, whereas the extension products containing 5 ' biotin are insensitive to the exonuclease over a wide range of nuclease concentrations.
- pairs of single-stranded amplification primers are obtained, which consist of a 5 ' end part, derived from the linker sequence that was added to the cloning vector by linker ligation, and a 3 ' end part, derived from ends of the inserts cloned into the vector.
- Fig. 1A, part C there is located immediately upstream of these 16 bases in the primers a dinucleotide, AG, representing the last two positions in the recognition sequence for the enzyme Gsul. These positions are also known to be present in the genomic DNA from which the cloned fragment was derived since these fragments were derived by digestion with the blunt end generating restriction enzyme Alul (Fig. 1A, part C) .
- Each one of the enzyme-synthesized primers therefore has a number (here 18) of bases (the 3' end bases plus two of the 5' end bases) that are complementary to the genomic sequence at each side of the cloned fragment, and a number of bases derived from the vector.
- the above enzymatically synthesized primers may be used for PCR amplification of a fragment obtained by Alul digestion of chromosomal DNA as schematically illustrated in Fig. IB, part D.
- the primers are used in a number of, say 5, amplification cycles, when necessary using a long annealing time to compensate for relatively low concentration of enzyme-synthesized primers.
- the desired DNA fragments are obtained, flanked at either end by the vector sequence. It is then no longer necessary to use the enzymatically synthesized primers, but the further amplification of the fragments to large numbers may conveniently be performed with the "standard" vector- derived primer, i.e one of the linker primers or a variant thereof.
- a cloning vector is prepared which contains the two recognition sites for the asymmetrically cleaving enzyme immediately adjacent each other but in opposite orientations and together containing the recognition site for a bluntly cleaving restriction enzyme, such that the enzyme may cleave right between the two sites.
- the steps of the present pr- dure are simple and may easily be performed for a la-L ; number of fragments in parallel, permitting the development of large sets of genetic markers.
- successful markers may be sequenced and converted to regular chemically synthesized PCR-based primers, but it is also possible to continue using enzyme-synthesized primers.
- Enzymatically synthesized amplification primers, constructed as described above, can also provide highly specific and sensitive detection reagents.
- amplification primers suitable to detect individual organisms in complex mixtures by PCR may be obtained by restriction digesting DNA preparations, cloning the fragments into the specialized vector described above, and isolating individual clones in order to generate a desired number of pairs of amplification primers. These amplification primers may thus be developed and tested without any requirement for access to DNA samples from isolated organisms or for DNA sequence information from these.
- nested PCR a number of cycles are conducted with a first set of primers, whereupon a number of cycles are run with a second set of primers hybridizing internally of the first primer set. This increases the efficiency and selectivity of the PCR process.
- end fragments may be efficiently isolated by amplifying the cloned fragments in two separate reactions as follows:
- one or the other amplification primer is biotinylated, permitting the amplified molecules to be isolated on a solid support, such as streptavidin-coated combs, e.g. of the type described in WO 94/11529, or paramagnetic particles. Other means of immobilization including DNA ligation may also be used.
- a solid support such as streptavidin-coated combs, e.g. of the type described in WO 94/11529, or paramagnetic particles.
- Other means of immobilization including DNA ligation may also be used.
- one or the other of the end fragments are released from the rest of the amplified molecules by selectively digesting the asymmetric restriction enzyme site located at the end remote from the support. This selective digestion may be achieved by using vectors with recognition sequences for two different asymmetric restriction enzyme sites, e.g.
- type IV enzymes on each side of the cloned inserts and cleaving the immobilized, amplified molecules in two separate reactions.
- Examples of such pairs of type IV restriction enzymes are Gsul and Eco57l.
- vectors with a single restriction site on both sides of the insert may be used if the biotinylated amplification primers are designed such that they are mismatched to the vector in e.g. positions 5 and 6 in from the 3' end of the primer, corresponding to the first 2 bases of the 6 base recognition sequence of a type IV restriction enzyme.
- Other sequence alterations are, of course, also possible, preserving the ability of the primers to amplify the cloned fragment but destroying the recognition sequence for one or the other of the sites.
- the two amplification products may be pooled before immobilization on the supports and restriction cleavage. After cleavage, released fragments are treated with ⁇ -exonuclease to obtain single stranded probes, and may then be directly used as enzymatic amplification primers.
- the enzymatic primer synthesis approach of the invention may also be used for producing circularizable probes.
- circularizable probes so-called "padlock" probes
- Such probes consist of two target-complementary segments, connected by a linker sequence.
- a linker sequence Upon recognition of a specific nucleic acid molecule, the ends of the probe are joined through the action of a ligase, creating circular DNA molecules catenated to the target sequence.
- such a circularizable probe may be prepared by cloning a DNA sequence into a specially designed vector, and the vector may then be used as a circularizable probe without the use of DNA sequence information from the cloned fragment, or the use of specific oligonucleotides.
- a large set of such clones may be processed in parallel for e.g. subtractive comparisons between cDNA populations.
- library to library comparisons may be made between for instance a library of all genes expressed in a given tissue and on the other hand all sequences located in a particular region of the genome, from yeast artificial chromosomes, subcloned in a circular single stranded plasmid library. This is, for example, useful when a disease gene has been located to a region by linkage analysis and it is known to be expressed in a particular tissue.
- the necessary vector may be prepared by ligating oligonucleotides to a restriction digested plasmid to generate, on one hand, a recognition motif for an asymmetrically cleaving enzyme, such as Gsul, and, on the other hand, a nearby situated rare restriction site, such as Notl.
- asymmetrically cleaving enzyme such as Gsul
- a nearby situated rare restriction site such as Notl.
- One way of constructing the vector is by inserting two oligonucleotide dimers to two different ends, generated by digestion with two restriction enzymes. Recombinant molecules are then produced by ligating blunt end DNA fragments, e.g. generated by Alul digestion, to the vector. The constructs obtained are - ransformed into bacteria and single-stranded recombinant molecules are generated.
- a primer is hybridized to the vector molecule and extended using a DNA polymerase, rendering the recognition sequence for the asymmetrically cleaving enzyme double stranded and permitting cleavage of the insert. After digestion of the molecules with the enzyme, the fragments of extended molecules are removed by denaturing washes.
- the immobilized circularizable probes obtained may be used for trapping target molecules, as is also illustrated in Fig. 2.
- a population of recombinant clones prepared as above is turned into single-stranded circular molecules.
- this library should, of course, be of the opposite polarity to the above construct.
- the vector must not have the same rare-cutter enzyme site or at least not the same polarity of the sequence surrounding the recognition sequence.
- oligonucleotide is then annealed to the region of the rare-cutter side on the capture vectors, and these are linearized by digestion with the rare cutter enzyme. Trapped clones are released by denaturing washes, repaired, and transformed into bacteria for molecular cloning.
- Control primer Al 5' AATTG ACCGT TAGCA ACTGG AGCTC AGCAG CCCGT GAT 3 ' - Control primer AMI: 5' CTC AGCAG CCCGT GAT 3'
- Plasmid pBLUESCRIPT M13 was digested with EcoRI and, in the same reaction, the oligonucleotide duplex Omnil and Omni2 were ligated to the restriction fragment ends (Fig. 1A, part A) .
- 20 U of EcoRI were added to 5 ⁇ g of the plasmid in a final volume of 10 ⁇ l containing 10 mM Tris- HCl, pH 7.5, 10 mM MgCl2/ 50 mM potassium acetate, and 5 mM ATP.
- 2.5 U of T4 D ⁇ A ligase were added with oligonucleotides Omnil and Omni2 at 25 ⁇ M each.
- the reaction was left at 14°C over-night.
- Linearized vector molecules with added linkers were gel purified in a 1.5% ⁇ uSieve GTG agarose gel ( ⁇ algene) , and used as a cloning vector.
- the digestion products were separated by electrophoresis in a 2% agarose gel. End fragments released from the amplification products by enzymatic digestion were isolated from the gel, taking care not to contaminate the material with undigested material.
- Amplification using enzvme-svnthesized primers Enzymatically synthesized primers were used at a concentration of 0.05 ⁇ M, together with oligonucleotide Omnil at 1 ⁇ M, for amplification of human genomic DNA samples (Fig. IB, part D) . During the first 5 amplification cycles, annealing times were set at 10 minutes followed by a regular amplification protocol. Since the melting temperatures are not known for the template-specific 3 ' - ends of the amplification primers, two different different amplification programs were tried for each primer pair.
- the complete amplification program was as follows: 5 cycles of 94°C for 1 minute, annealing at 40°C or 55°C for 5-15 minutes, and 72°C for 1 minute, followed by 30 cycles of 94 °C for 1 minute, 55°C for 1 minute, and 72°C for 1 minute.
- FIG. 3 illustrates agarose gel electrophoresis of the results of amplification reactions using either chemically synthesized, 16 bases long primers (Ami and Am2) , lane 2 and lane 3 (without template); the same 16 bases with additionally 22 bases at the 5 ' ends identical to Omnil (Al and A2) , lane 4 and lane 5 (without template) ; amplification with BOmnil from the plasmid clone used to generate the primers, lane 6 and lane 7 (without template) ,* or enzyme-synthesized primers for a 200 bases long Alul fragment of known DNA sequence, assumed to be identical in sequence to oligonucleotides Al and A2, lane 8 and lane 9 (without template) .
- Lanes 1 and 10 are 100 bp ladders. As appears from the autoradiograph, all three pairs of oligonucleotides, when applied to human genomic DNA samples, gave rise to amplification products of approximately the same size. This is the size expected for these primers. In the absence of added template DNA, no amplification products were observed, affirming that the amplification products did not represent copies of contaminating undigested amplified clone inserts. Identification of polymorphic sequences The amplification primer Omnil was kinased with 32p in a 30-minute reaction at 37°C in 50 mM Tris-HCl, pH 7.5, 50 mM KC1, 10 mM MgCl2» and 0.5 ICI ⁇ 32 P ATP. The primer was used for amplification of genomic DNA samples, followed by separation of the products by 6% polyacrylamide denaturing gel electrophoresis. Size variation among amplification products was revealed by autoradiography.
Abstract
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Priority Applications (3)
Application Number | Priority Date | Filing Date | Title |
---|---|---|---|
JP8515251A JPH10508483A (en) | 1994-11-07 | 1995-11-07 | Methods for producing oligonucleotide probes or primers, vectors therefor and their use |
US08/836,222 US5952201A (en) | 1994-11-07 | 1995-11-07 | Method of preparing oligonucleotide probes or primers, vector therefor and use thereof |
EP95938100A EP0791057A1 (en) | 1994-11-07 | 1995-11-07 | Method of preparing oligonucleotide probes or primers, vector therefor and use thereof |
Applications Claiming Priority (2)
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SE9403805A SE9403805D0 (en) | 1994-11-07 | 1994-11-07 | Method of preparing oligonucleotide probes or primers, vector therefor and use thereof |
SE9403805-6 | 1994-11-07 |
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WO1996014406A1 true WO1996014406A1 (en) | 1996-05-17 |
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PCT/SE1995/001319 WO1996014406A1 (en) | 1994-11-07 | 1995-11-07 | Method of preparing oligonucleotide probes or primers, vector therefor and use thereof |
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US (1) | US5952201A (en) |
EP (1) | EP0791057A1 (en) |
JP (1) | JPH10508483A (en) |
CA (1) | CA2204637A1 (en) |
SE (1) | SE9403805D0 (en) |
WO (1) | WO1996014406A1 (en) |
Cited By (4)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US5871921A (en) * | 1994-02-16 | 1999-02-16 | Landegren; Ulf | Circularizing nucleic acid probe able to interlock with a target sequence through catenation |
US6566055B1 (en) * | 1996-09-19 | 2003-05-20 | Sequenom, Inc. | Methods of preparing nucleic acids for mass spectrometric analysis |
US9487823B2 (en) | 2002-12-20 | 2016-11-08 | Qiagen Gmbh | Nucleic acid amplification |
US9683255B2 (en) | 2005-09-09 | 2017-06-20 | Qiagen Gmbh | Method for activating a nucleic acid for a polymerase reaction |
Families Citing this family (4)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
WO1994003624A1 (en) * | 1992-08-04 | 1994-02-17 | Auerbach Jeffrey I | Methods for the isothermal amplification of nucleic acid molecules |
US6261808B1 (en) * | 1992-08-04 | 2001-07-17 | Replicon, Inc. | Amplification of nucleic acid molecules via circular replicons |
US6911307B1 (en) * | 1998-12-08 | 2005-06-28 | Proteus S.A. | Method of detection in vitro of a target substance in a sample comprising the labelling of said substance with a reporter gene and with the sequences necessary for the expression of said reporter gene in vitro |
WO2005113804A1 (en) * | 2004-05-20 | 2005-12-01 | Trillion Genomics Limited | Use of mass labelled probes to detect target nucleic acids using mass spectrometry |
Citations (1)
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WO1990001548A1 (en) * | 1988-07-29 | 1990-02-22 | Cancer Research Campaign Technology Limited | Gene modification |
Family Cites Families (14)
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JPS61501747A (en) * | 1984-04-06 | 1986-08-21 | ライフ テクノロジ−ズ インコ−ポレ−テツド | Method for detecting nucleic acid sequences |
US4883750A (en) * | 1984-12-13 | 1989-11-28 | Applied Biosystems, Inc. | Detection of specific sequences in nucleic acids |
US5242794A (en) * | 1984-12-13 | 1993-09-07 | Applied Biosystems, Inc. | Detection of specific sequences in nucleic acids |
AU622426B2 (en) * | 1987-12-11 | 1992-04-09 | Abbott Laboratories | Assay using template-dependent nucleic acid probe reorganization |
US5449602A (en) * | 1988-01-13 | 1995-09-12 | Amoco Corporation | Template-directed photoligation |
US4988617A (en) * | 1988-03-25 | 1991-01-29 | California Institute Of Technology | Method of detecting a nucleotide change in nucleic acids |
CA1341584C (en) * | 1988-04-06 | 2008-11-18 | Bruce Wallace | Method of amplifying and detecting nucleic acid sequences |
US5516663A (en) * | 1990-01-26 | 1996-05-14 | Abbott Laboratories | Ligase chain reaction with endonuclease IV correction and contamination control |
CA2049879A1 (en) * | 1990-08-30 | 1992-03-01 | Keith C. Backman | Controlled initial target-dependent production of templates for ligase chain reaction |
JP3080178B2 (en) * | 1991-02-18 | 2000-08-21 | 東洋紡績株式会社 | Method for amplifying nucleic acid sequence and reagent kit therefor |
US5426180A (en) * | 1991-03-27 | 1995-06-20 | Research Corporation Technologies, Inc. | Methods of making single-stranded circular oligonucleotides |
JP3085409B2 (en) * | 1991-03-29 | 2000-09-11 | 東洋紡績株式会社 | Method for detecting target nucleic acid sequence and reagent kit therefor |
SE9203320D0 (en) * | 1992-11-06 | 1992-11-06 | Pharmacia Lkb Biotech | A METHOD OF PROCESSING NUCLEIC ACID SAMPLES |
SE9400522D0 (en) * | 1994-02-16 | 1994-02-16 | Ulf Landegren | Method and reagent for detecting specific nucleotide sequences |
-
1994
- 1994-11-07 SE SE9403805A patent/SE9403805D0/en unknown
-
1995
- 1995-11-07 CA CA002204637A patent/CA2204637A1/en not_active Abandoned
- 1995-11-07 EP EP95938100A patent/EP0791057A1/en not_active Withdrawn
- 1995-11-07 JP JP8515251A patent/JPH10508483A/en active Pending
- 1995-11-07 WO PCT/SE1995/001319 patent/WO1996014406A1/en not_active Application Discontinuation
- 1995-11-07 US US08/836,222 patent/US5952201A/en not_active Expired - Fee Related
Patent Citations (1)
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WO1990001548A1 (en) * | 1988-07-29 | 1990-02-22 | Cancer Research Campaign Technology Limited | Gene modification |
Non-Patent Citations (1)
Title |
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GENE, Volume 54, 1987, R.B. GAYLE III ET AL., "Formation of MboII Vectors and Cassettes Using Asymmetric MboII Linkers", pages 221-228. * |
Cited By (5)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
US5871921A (en) * | 1994-02-16 | 1999-02-16 | Landegren; Ulf | Circularizing nucleic acid probe able to interlock with a target sequence through catenation |
US6235472B1 (en) | 1994-02-16 | 2001-05-22 | Ulf Landegren | Nucleic acid detecting reagent |
US6566055B1 (en) * | 1996-09-19 | 2003-05-20 | Sequenom, Inc. | Methods of preparing nucleic acids for mass spectrometric analysis |
US9487823B2 (en) | 2002-12-20 | 2016-11-08 | Qiagen Gmbh | Nucleic acid amplification |
US9683255B2 (en) | 2005-09-09 | 2017-06-20 | Qiagen Gmbh | Method for activating a nucleic acid for a polymerase reaction |
Also Published As
Publication number | Publication date |
---|---|
JPH10508483A (en) | 1998-08-25 |
CA2204637A1 (en) | 1996-05-17 |
US5952201A (en) | 1999-09-14 |
EP0791057A1 (en) | 1997-08-27 |
SE9403805D0 (en) | 1994-11-07 |
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